Chemical basis of glycine riboswitch cooperativity | Zendy

Miyun Kwon | Zendy; Scott A. Strobel | Zendy

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Chemical basis of glycine riboswitch cooperativity

Author(s) -

Miyun Kwon,

Scott A. Strobel

Publication year - 2007

Publication title -

rna

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 3.037

H-Index - 171

eISSN - 1469-9001

pISSN - 1355-8382

DOI - 10.1261/rna.771608

Subject(s) - cooperativity , riboswitch , aptamer , biology , helix (gastropod) , mutagenesis , nucleotide , glycine , biophysics , cooperative binding , rna , binding site , biochemistry , genetics , mutation , amino acid , gene , non coding rna , ecology , snail

The glycine binding riboswitch forms a unique tandem aptamer structure that binds glycine cooperatively. We employed nucleotide analog interference mapping (NAIM) and mutagenesis to explore the chemical basis of glycine riboswitch cooperativity. Based on the interference pattern, at least two sites appear to facilitate cooperative tertiary interactions, namely, the minor groove of the P1 helix from aptamer 1 and the major groove of the P3a helix from both aptamers. Mutation of these residues altered both the cooperativity and binding affinity of the riboswitch. The data support a model in which the P1 helix of the first aptamer participates in a tertiary interaction important for cooperativity, while nucleotides in the P1 helix of the second aptamer interface with the expression platform. These data have direct analogy to well-characterized mutations in hemoglobin, which provides a framework for considering cooperativity in this RNA-based system.

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